Lecture 36: Cortical Circuits 3

Question 1

What are the advantages of in vitro systems over in vivo systems when it comes to the study of neurophysiology and neuronal function?

Answer 1

can examine specific subsets of cells in isolation, simplified system, allows you to manipulate neuronal biology, exquisite temporal and spatial resolution, comparatively higher throughput (allows you to directly compare many variables in parallel)

Question 2

What are the common in vitro systems for studying neuronal function?

Answer 2

primary neuronal culture, iPSCs and organoids

Question 3

What is primary neuronal culture?

Answer 3

cells (neurons) taken from animal tissue and grown in supportive nutrient media in an incubator

Question 4

How is a primary neuronal culture made?

Answer 4

collect rodent embryos or early postnatal pups -> remove the brain -> separate the cortical hemispheres -> remove meninges, microdissection to isolate the brain region of interest -> enzymatic digestion of tissue and trituration to separate cells into single cell suspension -> cells plated down and grown in supportive nutrient media

Question 5

What are the strengths of primary neuronal culture?

Answer 5

relatively inexpensive, can be used in a high throughput manner, neurons mature quickly, easy to control, can be cultured from transgenic rodents, can culture cells from different brain regions, easy to assess synaptic function

Question 6

What are the limitations of primary neuronal culture?

Answer 6

simplified system (monolayer), neurons lose their normal interconnectivity to different brain regions, cannot assess neural circuits (but can look at network activity)

Question 7

What are iPSC-derived neurons?

Answer 7

human neurons

induced pluripotent stem cells which are differentiate into specific neuronal subtypes

Question 8

How is the differentiation of iPSCs directed?

Answer 8

specific neuronal growth factors are added

Question 9

What are the strengths of iPSC-derived neurons?

Answer 9

can be programmed into many different types of neurons, amenable to high throughput screens, can be used for modelling human disease, can be gene-edited to study gene functions, can assess synaptic physiology

Question 10

What are the limitations of iPSC-derived neurons?

Answer 10

expensive, takes a long time to mature and to develop mature synapses (months), neurons lose their normal interconnectivity and circuitry, cannot assess neural circuits (but can look at network activity)

Question 11

What are organoids?

Answer 11

3D “mini-brains” derived from iPSCs

display structures that resemble defined brain regions

Question 12

How are organoids generated?

Answer 12

embryoid bodies derived from iPSCs are generally embedded into an extracellular matrix and then cultivated in a rotating bioreactor to promote amplification and neural differentiation

Question 13

What are the strengths of organoids?

Answer 13

can be used to develop distinct brain structures which possess some of the layering that is found in the human brain, huge potential for modelling human disease and neurodevelopment, can be gene-edited to study gene function, can assess network activity and simple circuits

Question 14

What are the limitations of organoids?

Answer 14

very expensive, takes a very long time to develop (months), have a limited maturation, significant issues with cell death due to limited oxygen and nutrient diffusion, batch effects and heterogeneity, cannot assess complex neural circuits

Question 15

How can neuronal cultures be used?

Answer 15

can be used for a variety of different assays to assess cellular function and synaptic physiology

Question 16

What can in vitro systems be transfected or transduced to express?

Answer 16

genes / protein of interest
fluorescent reporters of neuronal activity
receptors that enable modulation of neuronal activity e.g. DREADDS

Question 17

What is the purpose of immunolabeling and fluorescence microscopy?

Answer 17

allows neuroscientists to assess expression and localization of proteins, or visualise organelles (eg microtubules, mitochondria, lysosomes)

Question 18

What is super-resolution imaging?

Answer 18

imaging beyond the diffraction limit (imposed by the diffraction of light)

Question 19

What does super-resolution imaging allow for?

Answer 19

resolution of single particles (e.g. movement of single proteins in different neuronal compartments)

Question 20

What is a strength of using neurons in culture?

Answer 20

easy to assess neuronal activity and synaptic physiology at the level of a single synapse

Question 21

What does live cell imaging allow?

Answer 21

allows neuroscientists to measure neurotransmitter release and synaptic vesicle dynamics in individual synapses, or populations of synapses

Question 22

What is an example of population level data?

Answer 22

how does a drug affect the amount of neurotransmitter available in neurons?

Question 23

What is an example of single cell data?

Answer 23

what is the difference in mRNA content between excitatory and inhibitory neurons?

Question 24

What are the several options for studying synaptic physiology?

Answer 24

patch clamping (electrophysiological assay)
multi-electrode arrays
voltage sensing dyes
Ca2+ imaging

Question 25

What is Baker-Gordon Syndrome?

Answer 25

a rare neurodevelopmental disorder caused by mutations to the SYT1 gene

Question 26

What are symptoms of Baker-Gordon Syndrome?

Answer 26

developmental delay, intellectual disability, movement disorder, behavioural outbursts, altered brain activity

Question 27

What does the SYT1 gene encode?

Answer 27

synaptotagmin 1, an essential presynaptic protein that plays a critical role in synaptic transmission

Question 28

Where is synaptotagmin 1 highly expressed?

Answer 28

in the cortex, hippocampus, midbrain and striatum/basal ganglia

Question 29

What is the role of synaptotagmin 1?

Answer 29

is the Ca2+ sensor for action-potential evoked neurotransmitter release

Question 30

What is the role of the primary antibody in immunolabeling?

Answer 30

will recognise all synaptotagmin (endogenous and transfected)

Question 31

What is the role of the secondary antibody in immunolabeling?

Answer 31

will recognise the primary antibody, and is conjugated to a red fluorescent tag

Question 32

What is the role of the green fluorescence in immunolabeling?

Answer 32

the presence of a GFP tag allows for tracking of transfected neurons (because not all neurons will be transfected)

Question 33

How do mutations to synaptotagmin 1 impact the expression of the protein?

Answer 33

the M303K mutation impaired the stability and expression of synaptotagmin 1; all other mutations had no effect

Question 34

What do mutations in synaptotagmin 1 affect?

Answer 34

the stability and expression level of synaptotagmin (M303K) OR have dominant-negative effects on the rate of exocytosis in a GRADED manner

Question 35

What is the result of there being a correlation between genotype and phenotypic spectrum?

Answer 35

those variants which have the greatest impact on rate of exocytosis are present in patients with the most severe phenotype